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两种甲苯胺蓝O介导的脱氧核糖核酸酶检测技术的改进

Improvement of two toluidine blue O-mediated techniques for DNase detection.

作者信息

Waller J R, Hodel S L, Nuti R N

出版信息

J Clin Microbiol. 1985 Feb;21(2):195-9. doi: 10.1128/jcm.21.2.195-199.1985.

DOI:10.1128/jcm.21.2.195-199.1985
PMID:3972986
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC271612/
Abstract

Two DNase detection techniques in which the metachromatic dye toluidine blue O (TBO) is used have been improved, and a potential source of difficulty for personnel attempting to use TBO-related methods has been identified. Reducing the concentration of TBO in the Streitfeld plate-flooding method from 0.1 to 0.05% resulted in easier control of staining intensity, less masking of DNase-positive reactions due to overstaining, sharper delineation of zones of DNase activity, and more sensitive detection of weak DNase reactions. Incorporation of 0.005% TBO in DNase agar, rather than the recommended 0.01%, allowed growth and expression of DNase activity by gram-positive as well as gram-negative bacteria. The reduced dye content in the agar also enhanced expression of DNase activity by some organisms and provided sharper delineation of DNase-positive reactions. Because optimum expression of DNase activity depends upon exact TBO concentrations in both the flooding and agar incorporation techniques, strict attention must be paid to the dye content of commercially available TBO dye powders. TBO concentrations must reflect actual dye content; therefore, calculations must include a conversion factor that accounts for the true dye content of the commercial preparation. The conversion factor that we developed is determined by dividing 100 by the percentage of dye in the commercial powder. The grams of commercial dye powder required per 100 ml of dye mixture is calculated by multiplying the percentage of dye required in the dye mixture by the conversion factor.

摘要

两种使用异染染料甲苯胺蓝O(TBO)的脱氧核糖核酸酶(DNase)检测技术得到了改进,并且已经确定了试图使用与TBO相关方法的人员可能遇到困难的一个潜在来源。在施特赖特费尔德平板灌注法中,将TBO的浓度从0.1%降至0.05%,使得染色强度更易于控制,减少了因过度染色导致的DNase阳性反应的掩盖,DNase活性区域的 delineation更清晰,并且对微弱DNase反应的检测更灵敏。在DNase琼脂中加入0.005%的TBO,而不是推荐的0.01%,使得革兰氏阳性菌和革兰氏阴性菌都能生长并表达DNase活性。琼脂中降低的染料含量也增强了一些生物体的DNase活性表达,并使DNase阳性反应的 delineation更清晰。由于DNase活性的最佳表达取决于灌注法和琼脂掺入法中确切的TBO浓度,因此必须严格注意市售TBO染料粉末的染料含量。TBO浓度必须反映实际染料含量;因此,计算必须包括一个考虑商业制剂真实染料含量的转换因子。我们开发的转换因子是通过将100除以商业粉末中染料的百分比来确定的。每100毫升染料混合物所需商业染料粉末的克数是通过将染料混合物中所需染料的百分比乘以转换因子来计算的。

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本文引用的文献

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Evaluation of extracellular deoxyribonuclease activity in Pseudomonas.铜绿假单胞菌细胞外脱氧核糖核酸酶活性的评估
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Metachromatic agar-diffusion methods for detecting staphylococcal nuclease activity.用于检测葡萄球菌核酸酶活性的异染琼脂扩散法。
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